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  • Showing results for necrosis-avid[Title] AND small[Title] AND molecule[Title] AND HQ4-DTPA[Title] AND multimodal[Title] AND imaging[Title] AND agent[Title] AND monitoring[Title] AND radiation[Title] AND tumor[Title] AND cell[Title] AND death[Title]. Your search for The necrosis-avid small molecule HQ4-DTPA as a multimodal imaging agent for monitoring radiation therapyinduced tumor cell death retrieved no results.
Front Oncol. 2016 Oct 21;6:221. eCollection 2016.

The Necrosis-Avid Small Molecule HQ4-DTPA as a Multimodal Imaging Agent for Monitoring Radiation Therapy-Induced Tumor Cell Death.

Author information

1
Department of Radiology, Leiden University Medical Center, Leiden, Netherlands; Percuros BV, Enschede, Netherlands.
2
Princess Margaret Cancer Center, University Health Network, Toronto, ON, Canada; Department of Medical Biophysics, University of Toronto, Toronto, ON, Canada.
3
Princess Margaret Cancer Center, University Health Network , Toronto, ON , Canada.
4
STTARR Innovation Centre, University Health Network , Toronto, ON , Canada.
5
LCBIM, Institute of Chemical Sciences and Engineering, Swiss Federal Institute of Technology of Lausanne (EPFL) , Lausanne , Switzerland.
6
Department of Radiology, Leiden University Medical Center , Leiden , Netherlands.
7
Percuros BV , Enschede , Netherlands.
8
Department of Radiology, Erasmus Medical Center , Rotterdam , Netherlands.
9
Princess Margaret Cancer Center, University Health Network, Toronto, ON, Canada; Department of Medical Biophysics, University of Toronto, Toronto, ON, Canada; Techna Institute, University Health Network, Toronto, ON, Canada.

Abstract

PURPOSE:

Most effective antitumor therapies induce tumor cell death. Non-invasive, rapid and accurate quantitative imaging of cell death is essential for monitoring early response to antitumor therapies. To facilitate this, we previously developed a biocompatible necrosis-avid near-infrared fluorescence (NIRF) imaging probe, HQ4, which was radiolabeled with 111Indium-chloride (111In-Cl3) via the chelate diethylene triamine pentaacetic acid (DTPA), to enable clinical translation. The aim of the present study was to evaluate the application of HQ4-DTPA for monitoring tumor cell death induced by radiation therapy. Apart from its NIRF and radioactive properties, HQ4-DTPA was also tested as a photoacoustic imaging probe to evaluate its performance as a multimodal contrast agent for superficial and deep tissue imaging.

MATERIALS AND METHODS:

Radiation-induced tumor cell death was examined in a xenograft mouse model of human breast cancer (MCF-7). Tumors were irradiated with three fractions of 9 Gy each. HQ4-DTPA was injected intravenously after the last irradiation, NIRF and photoacoustic imaging of the tumors were performed at 12, 20, and 40 h after injection. Changes in probe accumulation in the tumors were measured in vivo, and ex vivo histological analysis of excised tumors was performed at experimental endpoints. In addition, biodistribution of radiolabeled [111In]DTPA-HQ4 was assessed using hybrid single-photon emission computed tomography-computed tomography (SPECT-CT) at the same time points.

RESULTS:

In vivo NIRF imaging demonstrated a significant difference in probe accumulation between control and irradiated tumors at all time points after injection. A similar trend was observed using in vivo photoacoustic imaging, which was validated by ex vivo tissue fluorescence and photoacoustic imaging. Serial quantitative radioactivity measurements of probe biodistribution further demonstrated increased probe accumulation in irradiated tumors.

CONCLUSION:

HQ4-DTPA has high specificity for dead cells in vivo, potentiating its use as a contrast agent for determining the relative level of tumor cell death following radiation therapy using NIRF, photoacoustic imaging and SPECT in vivo. Initial preclinical results are promising and indicate the need for further evaluation in larger cohorts. If successful, such studies may help develop a new multimodal method for non-invasive and dynamic deep tissue imaging of treatment-induced cell death to quantitatively assess therapeutic response in patients.

KEYWORDS:

cancer; cell death; cyanine; fluorescence imaging; multimodal imaging; necrosis avid contrast agent; radiation therapy; treatment response

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